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评估铀酰光裂解作为监测RNA中离子结合和柔性的探针。

Evaluation of uranyl photocleavage as a probe to monitor ion binding and flexibility in RNAs.

作者信息

Wittberger D, Berens C, Hammann C, Westhof E, Schroeder R

机构信息

Institute of Microbiology and Genetics, Vienna Biocenter, University of Vienna, Dr. Bohrgasse 9, A-1030 Vienna, Austria.

出版信息

J Mol Biol. 2000 Jul 7;300(2):339-52. doi: 10.1006/jmbi.2000.3747.

Abstract

In order to evaluate uranyl photocleavage as a tool to identify and characterize structural and dynamic properties in RNA, we compared uranyl cleavage sites in five RNA molecules with known X-ray structures, namely the hammerhead and hepatitis delta virus ribozymes, the P4-P6 domain of the Tetrahymena group I intron, as well as tRNA(Phe) and tRNA(Asp) from yeast. Uranyl photocleavage was observed at specific positions in all molecules investigated. In order to characterize the sites, photocleavage was performed in the absence and in increasing amounts of MgCl(2). Uranyl photocleavage correlates well with sites of low calculated accessibility, suggesting that uranyl ions bind in tight RNA pockets formed by close approach of phosphate groups. RNA foldings require ion binding, usually magnesium ions. Thus, upon the adoption of the native structure, uranyl ions can no longer bind well except in flexible and open to the solvent regions that can undergo induced-fit without disrupting the native fold. Uranyl photocleavage was compared to N-ethyl-N-nitrosourea and lead-induced cleavages in the context of the three-dimensional X-ray structures. Overall, the regions protected from ENU attack are sites of uranyl cleavage, indicating sites of low accessibility which can form ion binding sites. On the contrary, lead cleavages occur at flexible and accessible sites and correlate with the unspecific cleavages prevalent in dynamic and open regions. Applied in a magnesium-dependent manner, and only in combination with other backbone probing agents such as N-ethyl-N-nitrosourea, lead and Fenton cleavage, uranyl probing has the potential to reveal high-affinity metal ion environments, as well as regions involved in conformational transitions.

摘要

为了评估铀酰光裂解作为鉴定和表征RNA结构及动力学特性的工具,我们比较了五个具有已知X射线结构的RNA分子中的铀酰裂解位点,即锤头状核酶和丁型肝炎病毒核酶、嗜热四膜虫I组内含子的P4-P6结构域,以及来自酵母的tRNA(Phe)和tRNA(Asp)。在所有研究的分子中均在特定位置观察到铀酰光裂解。为了表征这些位点,在不存在MgCl₂以及MgCl₂含量不断增加的情况下进行光裂解。铀酰光裂解与计算得出的低可及性位点密切相关,这表明铀酰离子结合在由磷酸基团紧密靠近形成的紧密RNA口袋中。RNA折叠需要离子结合,通常是镁离子。因此,在采用天然结构后,除非在可灵活开放至溶剂区域且可发生诱导契合而不破坏天然折叠的情况下,铀酰离子无法再很好地结合。在三维X射线结构的背景下,将铀酰光裂解与N-乙基-N-亚硝基脲和铅诱导的裂解进行了比较。总体而言,免受ENU攻击的区域是铀酰裂解位点,表明这些位点可及性低,能够形成离子结合位点。相反,铅裂解发生在灵活且可及的位点,并且与动态和开放区域中普遍存在的非特异性裂解相关。以镁依赖的方式应用,并且仅与其他主链探测剂(如N-乙基-N-亚硝基脲、铅和芬顿裂解)结合使用时,铀酰探测有潜力揭示高亲和力金属离子环境以及参与构象转变的区域。

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